Assessment and validation of the MS/MS fragmentation patterns of the macrolide immunosuppressant everolimus

Boernsen, K. Olaf; Egge-Jacobsen, Wolfgang; Inverardi, Bruno; Strom, Tobin; Streit, Frank; Schiebel, Hans‐Martin; Benet, Leslie Z.; Christians, Uwe

doi:10.1002/jms.1215

Cited by 32 publications

(43 citation statements)

References 22 publications

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“…15 The sirolimus metabolites were structurally identified based on detailed analysis of their MS/MS and MS n fragmentation patterns as previously described. 16 Key assay performance parameters for sirolimus were as follows: lower limit of quantitation, 0.1 ng/mL; range of linear response, 0.1-100 ng/mL (r . 0.99, n = 6); mean absolute recovery during extraction, 87.3%; total imprecision, 6.7%-9.8%; and interday accuracy, 103.7%-108.0%.…”

Section: Lc-ms/ms Analysismentioning

confidence: 99%

Age-Dependent Changes in Sirolimus Metabolite Formation in Patients With Neurofibromatosis Type 1

Emoto

Fukuda

Mizuno

et al. 2015

Therapeutic Drug Monitoring

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Section: Lc-ms/ms Analysismentioning

confidence: 99%

Age-Dependent Changes in Sirolimus Metabolite Formation in Patients With Neurofibromatosis Type 1

Emoto

Fukuda

Mizuno

et al. 2015

Therapeutic Drug Monitoring

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“…The fragment ions of protonated ATG181 at m/z 532 and 829 (Fig. 2B) appeared to correspond to the Fragments a and C of everolimus at m/z 389 and 686 (Boernsen et al, 2007), differing from their precursor ions by 591 and 294 mass units, respectively. These two fragment ions and a few ions in the low mass region, all containing the trimethylammonium function, were the only ones observed in the product ion spectrum of protonated ATG181, in contrast to the product ion spectrum of sodiated everolimus, which showed fragment ions containing all parts of the molecule ( Fig.…”

Section: Resultsmentioning

confidence: 97%

The Macrolide Everolimus Forms an Unusual Metabolite in Animals and Humans: Identification of a Phosphocholine Ester

Zollinger¹,

Sayer²,

Dannecker³

et al. 2008

Drug Metab Dispos

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ABSTRACT:The immunosuppressant macrolide everolimus was found to be metabolized in animals and humans to a phosphocholine ester (ATG181), a hitherto unknown type of conjugate in xenobiotic metabolism. The structure of ATG181 was elucidated by mass spectrometry and confirmed by synthesis. ATG181 was among the most prominent metabolites of everolimus in rat, monkey, and human blood and was found also in various tissues of the rat, whereas no ATG181 was identified in the urine and feces of the species investigated. The metabolite showed binding to FK506 binding protein with a 2-to 3-fold higher affinity than everolimus. However, ATG181 exhibited only marginal in vitro immunosuppressive activity and is therefore very unlikely to contribute in a relevant manner to the immunosuppressive effect of everolimus.

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“…Next the hydrogen from the methylene in the middle of aliphatic chain and carbonyl (colored in red), transfers to the oxygen of ester group via 1,3 hydrogen migration. Thereafter, the carbon (from aliphatic chain) - oxygen (from ester group) bond is broken, sequentially opening the loop and forming a carboxyl and ethylene at both ends respectively [24]–[28]. Finally, the compound, which loses water after ring opening, forms the [M-H-H 2 O] − ( m/z 1016).…”

Section: Resultsmentioning

confidence: 99%

The Specific Cleavage of Lactone Linkage to Open-Loop in Cyclic Lipopeptide during Negative ESI Tandem Mass Spectrometry: The Hydrogen Bond Interaction Effect of 4-Ethyl Guaiacol

et al. 2014

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Mass spectrometry is a valuable tool for the analysis and identification of chemical compounds, particularly proteins and peptides. Lichenysins G, the major cyclic lipopeptide of lichenysin, and the non-covalent complex of lichenysins G and 4-ethylguaiacol were investigated with negative ion ESI tandem mass spectrometry. The different fragmentation mechanisms for these compounds were investigated. Our study shows the 4-ethylguaiacol hydrogen bond with the carbonyl oxygen of the ester group in the loop of lichenysins G. With the help of this hydrogen bond interaction, the ring structure preferentially opens in lactone linkage rather than O-C bond of the ester-group to produce alcohol and ketene. Isothermal titration 1H-NMR analysis verified the hydrogen bond and determined the proportion of subject and ligand in the non-covalent complex to be 1∶1. Theoretical calculations also suggest that the addition of the ligand can affect the energy of the transition structures (TS) during loop opening.

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Assessment and validation of the MS/MS fragmentation patterns of the macrolide immunosuppressant everolimus

Cited by 32 publications

References 22 publications

Age-Dependent Changes in Sirolimus Metabolite Formation in Patients With Neurofibromatosis Type 1

Age-Dependent Changes in Sirolimus Metabolite Formation in Patients With Neurofibromatosis Type 1

The Macrolide Everolimus Forms an Unusual Metabolite in Animals and Humans: Identification of a Phosphocholine Ester

The Specific Cleavage of Lactone Linkage to Open-Loop in Cyclic Lipopeptide during Negative ESI Tandem Mass Spectrometry: The Hydrogen Bond Interaction Effect of 4-Ethyl Guaiacol

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